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分子轨迹揭示了油/水界面处蛋白质聚集和拥挤的特征。

Molecular trajectories provide signatures of protein clustering and crowding at the oil/water interface.

作者信息

McUmber Aaron C, Larson Nicholas R, Randolph Theodore W, Schwartz Daniel K

机构信息

Department of Chemical and Biological Engineering, University of Colorado Boulder, Boulder, Colorado 80309, United States.

出版信息

Langmuir. 2015 Jun 2;31(21):5882-90. doi: 10.1021/acs.langmuir.5b00984. Epub 2015 May 19.

DOI:10.1021/acs.langmuir.5b00984
PMID:25950404
Abstract

Using high throughput single-molecule total internal reflection fluorescence microscopy (TIRFM), we have acquired molecular trajectories of bovine serum albumin (BSA) and hen egg white lysozyme during protein layer formation at the silicone oil-water interface. These trajectories were analyzed to determine the distribution of molecular diffusion coefficients, and for signatures of molecular crowding/caging, including subdiffusive motion and temporal anticorrelation of the instantaneous velocity vector. The evolution of these properties with aging time of the interface was compared with dynamic interfacial tension measurements. For both lysozyme and BSA, we observed an overall slowing of protein objects, the onset of both subdiffusive and anticorrelated motion (associated with crowding), and a decrease in the interfacial tension with aging time. For lysozyme, all of these phenomena occurred virtually simultaneously, consistent with a homogeneous model of layer formation that involves gradual crowding of weakly interacting proteins. For BSA, however, the slowing occurred first, followed by the signatures of crowding/caging, followed by a decrease in interfacial tension, consistent with a heterogeneous model of layer formation involving the formation of protein clusters. The application of microrheological methods to single molecule trajectories described here provides an unprecedented level of mechanistic interpretation of interfacial events that occurred over a wide range of interfacial protein coverage.

摘要

我们使用高通量单分子全内反射荧光显微镜(TIRFM),获取了在硅油-水界面形成蛋白质层过程中牛血清白蛋白(BSA)和鸡蛋清溶菌酶的分子轨迹。分析这些轨迹以确定分子扩散系数的分布,以及分子拥挤/笼蔽的特征,包括亚扩散运动和瞬时速度矢量的时间反相关。将这些性质随界面老化时间的演变与动态界面张力测量结果进行了比较。对于溶菌酶和BSA,我们都观察到蛋白质物体整体变慢、亚扩散和反相关运动(与拥挤相关)的出现,以及界面张力随老化时间降低。对于溶菌酶,所有这些现象几乎同时发生,这与涉及弱相互作用蛋白质逐渐拥挤的层形成均匀模型一致。然而,对于BSA,变慢首先发生,接着是拥挤/笼蔽的特征,然后是界面张力降低,这与涉及蛋白质簇形成的层形成异质模型一致。此处描述的将微观流变学方法应用于单分子轨迹,为在广泛的界面蛋白质覆盖范围内发生的界面事件提供了前所未有的机制解释水平。

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